摘要
目的为建立有效的肿瘤治疗方法,筛查ODCmRNA最佳反义抑制位点。方法采用RT PCR的方法从肝癌细胞中扩增出鸟氨酸脱羧酶(ODC),外显子2、外显子3、外显子610、外显子11124段基因片段。通过TA克隆反向连接到pcDNA3.1上,酶切测序并鉴定插入方向。脂质体法转染重组载体及空载体到肝癌MMC7721细胞中,采用Western blot法检测各载体对ODC蛋白表达的抑制作用,采用四唑盐比色试验验证并比较各载体对MMC7721细胞增殖活性的影响。结果外显子2、外显子3、外显子6103个位点的ODC反义RNA表达载体转染细胞后,细胞内ODC蛋白表达量明显降低,细胞增殖活性受到明显抑制,抑制率分别为59%、62%、64%。结论ODC外显子2、外显子3、外显子610是较好的反义抑制敏感位点。
Objective :TO Screen the sensitive antisense targets in the ODCmRNA. Methods :Four parts of ODC gene which were extron2, extron3, extron6-10, extronll-12 were amplified from hepatic cancer cell by RT-PCR and then reversely subcloned into pcDNA3, i vector. Their inserted dlrections were identified by sequence. After transfecting the hepatic cancer cell line MMC7721 with these recombinant vectors and empty vectors pcDNA3, i, we adapted Western-blot and MTT assay to respectively identify and compare the effect of these vectors in the expression of OOC and cell growth, Results :Three ODC recombinant vectors of the best inhibi- tive effect were successfully selected. Conclusion :extron2, extron3 and extron6-10 were found to be the best antisense sites of inhibition.
出处
《中国现代普通外科进展》
CAS
2005年第3期146-150,共5页
Chinese Journal of Current Advances in General Surgery
基金
山东省科技厅发展计划项目
山东省卫生厅科研基金资助项目(2001CA1CAA3)
关键词
鸟氨酸脱羧酶
RNA
反义
真核表达载体
外显子
Ornithine decarboxylase RNA,antisense Eukaryotic expression vectors Exons
